pma诱导LFA-1和talin在完整克隆T辅助细胞中的特异性关联。

A Kupfer, P Burn, S J Singer
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引用次数: 0

摘要

先前对克隆T辅助细胞(Th)和抗原呈递细胞之间形成的单个细胞偶对的实验表明,细胞骨架蛋白talin可能与Th细胞中的细胞表面蛋白LFA-1相关。为了验证这一说法,我们用合适的特异性抗体试剂在完整的Th细胞上诱导LFA-1的表面盖层,然后通过双免疫荧光显微镜实验确定talin是否与LFA-1盖层共簇。在未处理的Th细胞中,LFA-1的封顶不会导致细胞内talin的重新分布。然而,如果用磷酸酯PMA处理完整的Th细胞,LFA-1的帽盖导致talin与LFA-1帽盖共同聚集,而不是α -肌动蛋白。无论是否使用PMA预处理,TCR或CD4在Th细胞上的封顶都不会导致talin与这些封顶共同聚集。因此,PMA处理Th细胞诱导talin与Th细胞表面下的LFA-1直接或间接结合。正如之前观察到的那样,PMA处理也增加了Th细胞的极化扩散和对基质的粘附。此外,我们发现,这种增加的pma治疗依从性被LFA-1抗体的存在所抑制。talin,很可能还有f -肌动蛋白微丝,与LFA-1的关联似乎介导了Th细胞黏附性的普遍增加。这些发现的相关性与分离的Th细胞Th细胞与特定抗原呈递细胞的相互作用进行了讨论。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
The PMA-induced specific association of LFA-1 and talin in intact cloned T helper cells.

Previous experiments with individual cell couples formed between cloned T helper (Th) cells and antigen-presenting cells have led us to suggest that the cytoskeletal protein talin may be associated with the cell surface protein LFA-1 in the Th cell. In order to examine this suggestion, we induced the surface capping of LFA-1 with suitable specific antibody reagents on the intact Th cells, and then determined by double immunofluorescence microscopic experiments, whether talin was co-clustered with the LFA-1 caps. With untreated Th cells, capping of LFA-1 did not result in any redistribution of intracellular talin. However, if the intact Th cells were treated with the phorbol ester PMA, the capping of LFA-1 resulted in a co-clustering of talin with the LFA-1 caps, but not a alpha-actinin. The capping of TCR or CD4 on the Th cells with or without pretreatment with PMA did not lead to any such co-clustering of talin with these caps. PMA treatment of the Th cells therefore induces a direct or indirect association of talin with LFA-1 underneath the Th cell surface. PMA treatment of the Th cells also increased their polarized spreading and adherence to substrata, as had been observed before. We found, furthermore, that this increased adherence upon PMA-treatment was inhibited by the presence of antibodies to LFA-1. The association of talin, and very likely also F-actin microfilaments, with LFA-1 appears to mediate a generalized increased adhesivity of the Th cells. The relevance of these findings with isolated Th cells to the interaction of Th cells with specific antigen-presenting cells is discussed.

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